The control of ATP synthesis in heart mitochondria : Functions of a naturally-occurring inhibitor protein

Jackson, P. J.

January 1987

No description available.

572

ATP synthesis in rat heart

Adenosine signaling in Drosophila / Adenosine signaling in Drosophila

KUČEROVÁ, Lucie

January 2013

This thesis characterizes adenosine signalization in Drosophila and describes response to adenosine in various cell types. Extracellular adenosine mediates most of its physiological effects through its receptors but recent data also indicate that adenosine transport also has important physiological functions. It was shown in this thesis that adenosine stimulates only cAMP second messenger system in Drosophila cells endogenously expressing AdoR. The pharmacological profile of the DmAdoR was established using the cAMP functional assay. The utility of the agonist 2-chloroadenosine and antagonist SCH58261 were examined in flies in vivo and compared with phenotypes of DmAdoR mutants. The responses of Drosophila cells to adenosine mediated by adenosine transport were also examined. Different cell types exhibited striking differences in adenosine uptake and adenosine recycling that were closely connected with the regulation of carbohydrate and lipid metabolism. This thesis provides an important foundation for the study of interactions between adenosine receptor and adenosine transport.

Altérations du métabolisme énergétique mitochondrial lors de la cachexie cancéreuse / Impairment of energetic mitochondrial metabolism in cancer cachexia

Julienne, Cloé Mimsy

17 February 2012

La cachexie est un syndrome complexe caractérisé par une balance énergétique négative. Le rôle joué par le métabolisme énergétique mitochondrial dans ce syndrome est peu connu. Nos précédents travaux montraient une diminution de la synthèse de l’ATP dans les mitochondries hépatiques en stade de cachexie cancéreuse sévère. Dans ce travail, nous démontrons, in vitro, que l’augmentation de la production d’espèce réactive de l’oxygène et du contenu en cardiolipine dans des mitochondries hépatiques saines, mime partiellement les mécanismes observés lors d’un stade cachexie sévère. Nous observons cependant que l’altération du métabolisme mitochondrial hépatique apparait à un stade tardif du développement de la cachexie. En stade sévère les mitochondries musculaires ne développent pas d’altération de leur efficacité de synthèse d’ATP mais une diminution des leurs capacités oxydatives. / Cancer cachexia is a composite syndrome, characterized by a negative energetic balance. The role played by mitochondrial energetic metabolism in this syndrome is poor known. Our past work showed a decrease of ATP synthesis efficiency in hepatic mitochondria in severe state of cancer cachexia. In this work, we demonstrate, in vitro, that increase of reactive oxygen species and cardiolipine content, in healthy mitochondria, can partly mimic the mechanisms observed in severe state of cancer cachexia. We observe that alteration of hepatic mitochondrial metabolism appear last during the development of cancer cachexia. In sever state of cancer cachexia, skeletal muscle mitochondria don’t develop this alteration but demonstrated a decrease of oxidative capacities.

Cachexie cancéreuse

Mitochondrie

Synthèse d'ATP

Cardiolipine

Espèces réactives de l'oxygène

Cancer cachexia

Mitochondria

ATP synthesis

Cardiolipine

Reactive oxygen species

Dietary Bioflavonoids Inhibit Escherichia Coli ATP Synthase in a Differential Manner

Chinnam, Nagababu, Dadi, Prasanna K., Sabri, Shahbaaz A., Ahmad, Mubeen, Kabir, M. A., Ahmad, Zulfiqar

01 June 2010

The aim of this study was to determine if the dietary benefits of bioflavonoids are linked to the inhibition of ATP synthase. We studied the inhibitory effect of 17 bioflavonoid compounds on purified F1 or membrane bound F1Fo E. coli ATP synthase. We found that the extent of inhibition by bioflavonoid compounds was variable. Morin, silymarin, baicalein, silibinin, rimantadin, amantidin, or, epicatechin resulted in complete inhibition. The most potent inhibitors on molar scale were morin (IC50∼0.07mM)>silymarin (IC50∼0.11mM)>baicalein (IC50∼0.29mM)>silibinin (IC50∼0.34mM)>rimantadin (IC50∼2.0mM)>amantidin (IC50∼2.5mM)>epicatechin (IC50∼4.0mM). Inhibition by hesperidin, chrysin, kaempferol, diosmin, apigenin, genistein, or rutin was partial in the range of 40-60% and inhibition by galangin, daidzein, or luteolin was insignificant. The main skeleton, size, shape, geometry, and position of functional groups on inhibitors played important role in the effective inhibition of ATP synthase. In all cases inhibition was found fully reversible and identical in both F1Fo membrane preparations and isolated purified F1. ATPase and growth assays suggested that the bioflavonoid compounds used in this study inhibited F1-ATPase as well as ATP synthesis nearly equally, which signifies a link between the beneficial effects of dietary bioflavonoids and their inhibitory action on ATP synthase.

ATP synthesis

bioflavonoids

biological nanomotor

E. coli ATP synthase

F -ATPase 1

F F ATP synthase 1 o

Inhibition of ATPase Activity of Escherichia Coli ATP Synthase by Polyphenols

Dadi, Prasanna K., Ahmad, Mubeen, Ahmad, Zulfiqar

01 July 2009

We have studied the inhibitory effect of five polyphenols namely, resveratrol, piceatannol, quercetin, quercetrin, and quercetin-3-β-d glucoside on Escherichia coli ATP synthase. Recently published X-ray crystal structures of bovine mitochondrial ATP synthase inhibited by resveratrol, piceatannol, and quercetin, suggest that these compounds bind in a hydrophobic pocket between the γ-subunit C-terminal tip and the hydrophobic inside of the surrounding annulus in a region critical for rotation of the γ-subunit. Herein, we show that resveratrol, piceatannol, quercetin, quercetrin, or quercetin-3-β-d glucoside all inhibit E. coli ATP synthase but to different degrees. Whereas piceatannol inhibited ATPase essentially completely (∼0 residual activity), inhibition by other compounds was partial with ∼20% residual activity by quercetin, ∼50% residual activity by quercetin-3-β-d glucoside, and ∼60% residual activity by quercetrin or resveratrol. Piceatannol was the most potent inhibitor (IC50 ∼14 μM) followed by quercetin (IC50 ∼33 μM), quercetin-3-β-d glucoside (IC50 ∼71 μM), resveratrol (IC50 ∼94 μM), quercitrin (IC50 ∼120 μM). Inhibition was identical in both F1Fo membrane preparations as well as in isolated purified F1. In all cases inhibition was reversible. Interestingly, resveratrol and piceatannol inhibited both ATPase and ATP synthesis whereas quercetin, quercetrin or quercetin-3-β-d glucoside inhibited only ATPase activity and not ATP synthesis.

ATP synthesis

biological nanomotor

F -ATPase 1

F F -ATP synthase 1 o

piceatannol

polyphenols

quercetin

quercetin-3-β-d glucoside

quercitrin

resveratrol

Role of αPhe-291 Residue in the Phosphate-Binding Subdomain of Catalytic Sites of Escherichia Coli ATP Synthase

Brudecki, Laura, Grindstaff, Johnny J., Ahmad, Zulfiqar

15 March 2008

The role of αPhe-291 residue in phosphate binding by Escherichia coli F1F0-ATP synthase was examined. X-ray structures of bovine mitochondrial enzyme suggest that this residue resides in close proximity to the conserved βR246 residue. Herein, we show that mutations αF291D and αF291E in E. coli reduce the ATPase activity of F1F0 membranes by 350-fold. Yet, significant oxidative phosphorylation activity is retained. In contrast to wild-type, ATPase activities of mutants were not inhibited by MgADP-azide, MgADP-fluoroaluminate, or MgADP-fluoroscandium. Whereas, 7-chloro-4-nitrobenzo-2-oxa-1,3-diazole (NBD-Cl) inhibited wild-type ATPase essentially completely, ATPase in mutants was inhibited maximally by ∼75%, although reaction still occurred at residue βTyr-297, proximal to αPhe-291 in the phosphate-binding pocket. Inhibition characteristics supported the conclusion that NBD-Cl reacts in βE (empty) catalytic sites, as shown previously by X-ray structure analysis. Phosphate protected against NBD-Cl inhibition in wild-type but not in mutants. In addition, our data suggest that the interaction of αPhe-291 with phosphate during ATP hydrolysis or synthesis may be distinct.

ATP synthesis

biological nanomotor

catalytic sites

F -ATPase 1

F F -ATP synthase 1 0

nucleotide binding

oxidative phosphorylation

Pi-binding assays

Inhibition of <em>Escherichia coli</em> ATP Synthase by Polyphenols and Their Derivatives.

Dadi, Prasanna Keerthi

08 May 2010

We have studied the inhibitory effect of natural and structurally modified polyphenols on Escherichia coli ATP synthase to test (I) if the beneficial dietary effects of polyphenols are related to their inhibitory actions on ATP synthase, (II) if inhibitory effects of polyphenolic compound could be augmented through structural modifications, and (III) if they can act as antimicrobial agent through their actions on ATP synthesis. X-ray crystal structures of polyphenol binding sites suggested that polyphenols bind at a distinct polyphenol binding pocket, at the interface of α,β,γ-subunits. We found that both natural and modified polyphenols inhibit E. coli ATP synthase to varying degrees and structural modifications resulted in augmented inhibition. Inhibition was reversible in all cases. Both natural and modulated compounds inhibited E. coli cell growth to varying degrees. We conclude that dietary benefits of polyphenols may be in part due to the inhibition of ATP synthase.

resveratrol

polyphenols

E coli

F1Fo-ATP synthase

F1-ATPase

ATP synthesis

quercetin

biological nanomotor

quercetin-3-β-D glucoside

quercitrin

piceatannol

Bacteriology

Life Sciences

Microbiology

Molecular Modulation of a-Subunit VISIT-DG Sequence Residue Asp-350 in the Catalytic sites of <em>Escherichia coli</em> ATP Synthase.

Jonnalagadda, Sneha R

01 May 2011

ATP Synthase is the fundamental means of cellular energy production in animals, plants, and almost all microorganisms. In order to understand the mechanism of ATP catalysis, critical amino acid residues involved in Pi binding have to be identified. The αVISIT-DG sequence at the interface of α/β subunits that contains residues from 345-351 is highly conserved and αAsp-350 has been chosen because of its negative charge side chain and its close proximity (~2.8 Å) to the known phosphate binding residue αArg-376. The mutant's αD350R, αD350Q, αD350A, αR376A/D, and αG351R/A/D were generated by site directed mutagenesis and several biochemical assays were performed on them to understand the role played by the amino acid residues in Pi binding. Biochemical results suggest that αD350 may be involved in catalysis of ATP synthase and play an important role in Pi binding, whereas αG351 may be involved only in the structural integrity.

F1Fo- ATP Synthase

ATP Synthesis

E coli

biological nanomotor

VISIT-DG Sequence

NBD-Cl

Aluminum chloride

Scandium chloride

DCCD

DTT

Mg-ADP.

Life Sciences

Molecular Biology